人胎儿胸腺内bc1－2基因表达与分布

采用免疫酶组织化学与地高辛标记的单链ｃＤＮＡ探针原位杂交技术,研究了抗凋亡基因ｂｃｌ－２在人胎儿胸腺组织中的表达与分布。结果ｂｃｌ－２ｍＲＮＡ及其蛋白均优势定位于髓质区。提示胸腺中ｂｃｌ－２基因表达调控发生在转录水平;ｂｃｌ－２基因介导的细胞凋亡状态可能参与Ｔ淋巴细胞的成熟过程。     

慢性缺氧大鼠肺血管c-myc及bcl-2基因表达研究

应用免疫组织化学和Ｎｏｒｔｈｅｒｎ杂交方法,对慢性缺氧大鼠肺组织（主要是肺血管壁）原癌基因ｃ－ｍｙｃ和抗凋亡基因ｂｃｌ－２表达进行了研究。免疫组织化学观察提示,正常对照组大鼠肺血壁Ｃ－ｍｙｃ和Ｂｃｌ－２蛋白仅为弱阳性或不表达,慢性缺氧１、２周组大鼠肺血管壁这两种抗原表达比对照组显著增强,呈强阳性,Ｎｏｒｔｈｅｒｎ杂交结果表明：慢性缺氧１、２周组大鼠肺组织内ｃ－ｍｙｃ和ｂｃｌ－２的ｍＲＮＡ表达比对照组显著增加,以上结果提示,ｃ－ｍｙｃ及ｂｃｌ－２两种基因调节的细胞增殖与凋亡可能参与了慢性缺氧性肺动脉高压的发病进程。     

重组RA—538及反义c—myc腺病毒对人胃癌,食管癌和bcl—2高表达细胞系的作用

本课题研究ＲＡ５３８、反义c-ymc重组腺病毒对人胃癌（ＳＧＣ７９０１）、食管癌（Ｅ Ｃ１０９、ＥＣ８７１２）、正常人胚肺２ＢＳ（２ＢＳ）及ｂｃｌ－２高表达细胞第的体仙外生物学作用及其分子机制。结果显示Ａｄ－ＲＡ５３８及Ａｄ－ＡＳｃ－ｍｙｃ对ＳＧＣ７９０１细胞体内外均具有明显的生长抑制及凋亡诱导作用,并能抑制其ｃ－ｍｙｃ、ｂｃｌ－２、ｃｙｃｌｉｎＤ１基因的表达及刺激ｂａｘ基因的表达。对ＥＣ１０９、ＥＣ８     

bcl-2癌基因蛋白在甲状腺癌中的表达及其意义

利用免疫组织化学技术,对６４例甲状腺癌进行了ｂｃｌ－２蛋白表达的检测,同时进行ｐ５３蛋白的对照检测。结果显示,甲状腺癌中ｂｃｌ－２蛋白阳性表达率为８１．３％（５２／６４）,但未分化癌无阳性表达。ｐ５３蛋白在甲状腺癌的阳性表达率为２０．３％（１３／６４）,而未分化癌全部为阳性表达。两种抗体在甲状腺癌的阳性表达率有显著性差异（Ｐ＜０．０１）。结果提示ｂｃｌ－２蛋白在甲状腺癌的表达与肿瘤细胞的分化程度有关,并与ｐ５３蛋白呈反比关系,ｂｃｌ－２与ｐ５３蛋白表达的不同分布可作为判断甲状腺癌预后的一个重要参考指标     

核酶对bcl－2mRNA的体外切割

通过微机对ｂｃｌ－２ＲＮＡ二级结构的分析,设计针对ｂｃｌ－２片段５＇ＣＧＣＧＡＣＣＣＧＧＵＣＧＣＣＡＧＧＡＣＣＵＣＧ３＇的“锤头状”（Ｈａｍｍｅｒｈｅａｄ）核酶（Ｒｉｂｏｚｙｍｅ,ＲＤ）基因,平端连接于ｐＧＥＭ－３Ｚｆ（－）ＨｉｎｃⅡ位点,克隆后经测序表明序列正确,ｂｃｌ－２和Ｒｉｂｏｚｙｍｅ基因经体外转录,５０℃作用２ｈ,从１６５６－１６５７（Ｃ－Ｇ）位之间切断ｂｃｌ－２ＲＮＡ片段．     

细胞凋亡过程中bcl-2基因的甲基化

为探讨凋亡过程中,ｂｃｌ－２基因下调与该基因甲基化状态的关系,用５－氟尿嘧啶（５－Ｆｕ）诱导小鼠成纤维细胞ＮＣ３Ｈ１０,ＴＣ３Ｈ１０及人乳腺癌细胞ＭＣＦ－７的凋亡,分别检测了这三种细胞凋亡过程中ｂｃｌ－２的表达变化,与其调控区及编码区的甲基化状况．我们曾观察到５－Ｆｕ作用２４～４８ｈ出现细胞存活率下降,ＤＮＡ梯状断裂及细胞周期凋亡峰显现等典型凋亡现象．Ｎｏｒｔｈｅｒｎ杂交显示,在５－Ｆｕ作用１２ｈ时ｂｃｌ－２ｍＲＮＡ水平已明显降低．由此,我们用小鼠ｂｃｌ－２（ｍｂｃｌ－２）及人ｂｃｌ－２（ｈｂｃｌ－２）基因调控区ＰＣＲ扩增片段及ｂｃｌ－２编码区（ｃＤＮＡ）片段作为探针,与５－Ｆｕ作用１２ｈ的细胞ＤＮＡ的ＭｓｐⅠ／ＨｐａⅡ酶切产物进行Ｓｏｕｔｈｅｒｎ杂交,以未作用的细胞ＤＮＡ同样酶切杂交为对照．通过杂交带谱的变化,分析ｂｃｌ－２基因的甲基化状况．结果显示：ｍｂｃｌ－２及ｈｂｃｌ－２在５－Ｆｕ作用１２ｈ后调控区甲基化水平增高,但其编码区甲基化状态皆未出现可检出的变化．上述结果提示：ｂｃｌ－２基因调控区甲基化水平升高可能与该基因下调有关     

bcl－2基因家族对细胞凋亡的调节

ｂｃｌ－２基因为一原癌基因,因其在淋巴瘤和白血病中出现重排而得名。近年研究表明,ｂｃｌ－２基因是细胞凋亡的重要抑制基因,它的过度表达是癌症和自身免疫病发生的重要原因。最近又发现了几个与ｂｃｌ－２基因有不同程度同源性的调节基因,也在细胞凋亡中发挥作用。     

小鼠成纤维细胞凋亡过程中P53与bcl-2表达的时序性

为探讨细胞凋亡过程中,ｂｃｌ－２与Ｐ５３,这两种凋亡关键性基因的相互关系,用５－氟尿嘧啶（５－Ｆｕ）诱导小鼠正常与恶性转化的成纤维细胞的凋亡,观察了这两种基因在凋亡过程中表达变化的时序．经流式细胞计检测,这两种细胞在５－Ｆｕ作用２４ｈ均出现了凋亡峰,细胞存活率随之下降,ＤＮＡ电泳显现梯状断裂．Ｎｏｒｔｈｅｒｎ杂交结果显示,在５－Ｆｕ作用６ｈ后两种细胞Ｐ５３ｍＲＮＡ水平已明显增高,而ｂｃｌ－２ｍＲＮＡ水平则在作用１２ｈ方明显降低．Ｐ５３上调与ｂｃｌ－２下调的明显时序性,说明Ｐ５３具备作为ｂｃｌ－２基因负调控转录因子的条件．由此,为进一步了解凋亡过程的ｂｃｌ－２基因下调机理提供了线索     

反义bcl—2在胃癌细胞中的诱导表达及促凋亡作用

为了观察ｂｃｌ－２反义ＲＮＡ对胃癌细胞ＳＧＣ７９０１的促凋亡作用及ＭＴ－１１启动子的启动诱导活性,用分子克隆方法构建载体,以电泳术,电镜术,流式细胞术,原位杂交,裸鼠肿瘤抑制试验及化学发光分析等方法观察,结果表明,可诱导载体ｐＭＴｂＮ具有良好的诱导启动转录活性,Ｂｃｌ－２蛋白的表达下降使胃癌细胞ＳＧＣ７９０１更易发生凋亡,致瘤性也发生改变。     

Bcl——2基因表达对TNF及OA诱发的细胞编程死亡的不同效应

用ＴＮＦ和ＯＡ（Ｏｋａｄａｉｃａｃｉｄ）诱发人神经母细胞瘤ＳＫ细胞死亡,并证明细胞死亡为编程死亡（ＰｒｏｇｒｍｍｅｄＣｅｌｌＤｅａｔｈ,简称ＰＣＤ）。将编码Ｂｃｌ－２全长蛋白的ｃＤＮＡ植入ＰＪＸ４１ｎｅｏ载体中,使其表达由ＨＣＭＶ病毒起动子控制。形成的顺义（ｐＢｃｌ－２－Ｓ）及反义（ｐＢｃｌ－２－ＡＳ）表达质粒经转染导入ＳＫ细胞中获得稳定转染子。Ｗｅｓｔｅｒｎ印迹表明顺义转染子表达大量的２６ｋｄＢｃｌ－２蛋白,而反义转染子则不表达。增强表达的Ｂｃｌ－２蛋白能抑制由ＴＮＦ引发的ＰＣＤ,但不影响ＯＡ引发的ＰＣＤ,从而证明了Ｂｃｌ－２基因产物抗细胞死亡效应的特异性。     

Bcl-2 family gene modulation during spontaneous apoptosis of B-chronic lymphocytic leukemia cells

Malignant cell accumulation in B-cell chronic lymphocytic leukemia (B-CLL) is primarily caused by defective apoptosis rather than increased proliferation. To further understand the role of Bcl-2 family members, known regulators of apoptosis, in the abnormal B-CLL survival, we have measured their mRNA levels in fresh B-CLL cells and in cultures undergoing spontaneous apoptosis. Using RNA protection assays we found constitutive expression of most bcl-2 members with high levels of bcl2, bcl-w, bad, bak, bax, and the bcl-2/bax ratio, compared to normal PBL. Spontaneous apoptosis of B-CLL cells by in vitro culture resulted in decreased bcl-2, bcl-w, bfl-1, mcl-1, bak, bax, and bcl-2/bax expression. The pro-apoptotic member bik was only expressed in 5/19 cases and was not modulated during apoptosis, suggesting that bik is not involved in this process. Thus, several Bcl-2 family genes are regulated during B-CLL spontaneous apoptosis and their relative levels may contribute to in vivo progression of the disease.     

Prevention of hybridoma cell death by bcl-2 during suboptimal culture conditions

TB/C3 hybridoma cells were transected with either pEF-MClneopA or pEF bcl2-MClneopA vectors to produce a control cell line (TB/C3 pEF) and a cell line that overexpresses the "antiapoptotic" human bcl-2 protein (TB/C3 bcl2). Flow cytometry analysis of intracellular bcl-2 protein levels enabled near on-line monitoring of the stability of bcl-2 expression in the absence of drug selection. It was possible to maintain spontaneous selection of cells with the overexpression of bcl-2 protein during semicontinuous cultures at very low dilution rates, where cells were subjected to the selective conditions of nutrient limitation and high toxic metabolite concentrations. Interestingly, cells that overexpressed bcl-2 were adapted to suspension culture conditions significantly faster than control cells. Dual fluorescence staining with acridine orange and propidium iodide allowed for discrimination between viable, apoptotic, secondary necrotic, and necrotic cells, respectively. Compared with the usual trypan blue method of establishing culture viability, dual staining demonstrated that under stressful conditions a significant proportion of cells that excluded trypan blue were also undergoing cell death through apoptosis. In batch cultures the overexpression of bcl-2 more than doubled the membrane intact (MI) cell productive period (the integral of Ml cell density with respect to culture time) and increased the monoclonal antibody (mAb) production by approximately 40% when compared with the control cell line. The overexpression of bcl-2 protein also significantly extended the cell integrity and viability by the suppression of apoptosis in conditions of hypoxia, hyperoxia, glutamine deprivation, glucose deprivation, and serum limitation. The suppression of apoptosis in anaerobic conditions suggests that bcl-2 exerts its antiapoptotic activity by a mechanism that does not involve an oxidative reactive pathway. In conditions of excess thymidine, which suppressed cell proliferation, Ml cell density and specific mAb productivity were further enhanced by the overexpression of bcl-2, which suggests the possibility of accomplishing a controlled proliferation in immortalized cell lines without invoking cell death. Cell size and intracellular mAb were increased for TB/C3 bcl2 cells compared with TB/C3 pEF control cells when analyzed by flow cytometry. (c) 1997 John Wiley & Sons, Inc. Biotechnol Bioeng 54: 1-16, 1997.     

mdr-1和bcl-2基因在K562/ADM多药耐药细胞中的共表达

为探讨肿瘤细胞多药耐药(MDR)形成的分子机理,本文观察了mdr-1、bcl-2和bax基因及其编码蛋白在人红白血病细胞株K562/ADM中的可能共表达。结果显示,在K562/ADM细胞中,在以mdr-1及P-gp过度表达为 特征的MDR形成时,其bcl-2及产物Bcl-2也过度表达,其中Bcl-2的表达阳性率约为相应敏感株K562的11倍;而Bax在二种细胞中均呈阳性表达,但无显著差异(P>0.05),提示bcl-2基因在mRNA和蛋白水平上的过度表达可能是K562/ADM细胞MDR形成时细胞凋亡耐受的分子基础。     

Shift of the Cellular Oxidation-Reduction Potential in Neural Cells Expressing Bcl-2

Abstract: Expression of the protooncogene bcl-2 inhibits both apoptotic and in some cases necrotic cell death in many cell types, including neural cells, and in response to a wide variety of inducers. The mechanism by which the Bcl-2 protein acts to prevent cell death remains elusive. One mechanism by which Bcl-2 has been proposed to act is by decreasing the net cellular generation of reactive oxygen species. To evaluate this proposal, we measured activities of antioxidant enzymes as well as levels of glutathione and pyridine nucleotides in control and bcl-2 transfectants in two different neural cell lines—rat pheochromocytoma PC12 and the hypothalamic GnRH cell line GT1-7. Both neural cell lines overexpressing bcl-2 had elevated total glutathione levels when compared with control transfectants. The ratios of oxidized glutathione to total glutathione in PC12 and GT1-7 cells overexpressing bcl-2 were significantly reduced. In addition, the NAD⁺/NADH ratio of bcl-2 -expressing PC12 and GT1-7 cells was two- to threefold less than that of control cell lines. GT1-7 cells overexpressing bcl-2 had the same level of glutathione peroxidase, catalase, superoxide dismutase, and glutathione reductase activities as control cells. PC12 cells overexpressing bcl-2 had a twofold increase in superoxide dismutase and catalase activity when compared with matched control transfected cells. The levels of glutathione peroxidase and glutathione reductase in PC12 cells overexpressing bcl-2 were similar to those of control cells. These results indicate that the overexpression of bcl-2 shifts the cellular redox potential to a more reduced state, without consistently affecting the major cellular antioxidant enzymes.     

ANKHD1, ankyrin repeat and KH domain containing 1, is overexpressed in acute leukemias and is associated with SHP2 in K562 cells

In the present study, increased levels of ANKHD1 mRNA and protein expression in leukemia cell lines are reported, as compared with normal hematopoietic cells. Furthermore, a higher expression of ANKHD1 mRNA was detected in primary acute leukemia samples than in normal hematopoietic cells (P=0.002). ANKHD1 was detected in the cytosolic and membrane fraction of cells and was co-immunoprecipitated with SHP2 in protein extracts of K562 and LNCaP cell lines. These findings suggest a role for ANKHD1 as a scaffolding protein that may be associated with the abnormal phenotype of leukemia cells.